CN103255137B - A kind ofly detect the method for SKA1 genetic expression and the purposes of siRNA thereof - Google Patents
A kind ofly detect the method for SKA1 genetic expression and the purposes of siRNA thereof Download PDFInfo
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Abstract
The invention discloses a kind of siRNA suppressing SKA1 genetic expression, the length of described siRNA is 15 ~ 27bp.The invention also discloses the recombinant vectors containing this siRNA, this recombinant vectors transfecting eukaryotic cells, namely obtains the cell of SKA1 gene silencing.SiRNA sequence of the present invention can effectively be degraded the mRNA of SKA1 gene, thus specificity suppresses the expression of SKA1 gene.SiRNA of the present invention can be used for preparing the medicine comprising tumour with SKA1 gene-associated diseases; Simultaneously for the effect of research SKA1 gene in drug resistance of tumor, the clinical non-operative treatment of tumour particularly osteosarcoma, Colorectal cancer is had great importance.This invention also discloses the reverse transcription PCR primer that effectively can detect SKA1 from tissue or cell, and the application of this primer in diagnosing tumor.
Description
Technical field
The invention belongs to biological technical field, particularly the nucleotide sequence of a kind of siRNA suppressing SKA1 genetic expression, this siRNA and the recombinant vectors containing this siRNA coding DNA, and their purposes.The invention still further relates to the reverse transcriptase primer that effectively can detect SKA1 genetic expression from tissue or cell, and the application of this primer in diagnosing tumor.
Background technology
RNA interference refers to the gene silencing phenomenon brought out by double-stranded RNA, mainly through hindering the translation of specific gene or transcribing inhibition of gene expression.Research shows, length is siRNA molecule (the small interfering RNA of 21 ~ 23nt, siRNA) be the immediate cause (TuschlT causing RNA to disturb, Zamore PD, Sharp PA, Bartel DP.RNAi:double-stranded RNA directs theATP-dependent cleavage of mRNA at 21 to 23 nucleotide intervals.Cell 2000,101:25-33.).RNA interference has high efficiency, simplicity and specificity in inhibition of gene expression, has played vital role at present in gene functional research and disease treatment.In recent years, RNA interference had also achieved some achievements (Uprichard, Susan L.The therapeuticpotential of RNA interference.FEBS Letters 2005,579:5996-6007) in oncotherapy.
SKA1(The spindle and kinetochore associated complex subunit 1) assignment of genes gene mapping is in karyomit(e) 18q21.1, and coding is about the albumen of 30kDa containing 255 amino acid, molecular weight.At present the research of SKA1 protein structure is not also goed deep into; only specify that it has coiled-coil domain (Rual JF at N end; Venkatesan K; Hao T, et al.Towards a proteome-scale map of thehuman protein-protein interaction network.Nature 2005; 437:1173-1178.Sauer G, Korner R, Hanisch A, et al.Proteome analysis of the human mitotic spindle.MolCell Proteomics 2005; 4:35-43.).Initial mass spectrometry results shows; SKA1 albumen is confirmed as integral part (the Cheeseman IM of spindle body; Brew C; Wolyniak M, et al.Implicationof a novel multiprotein Dam1p complex in outer kinetochore function.J Cell Biol.2001; 155:1137-1145.).Afterwards by the two assorted test of yeast, find spindle body kinetochore mixture (The spindle and kinetochore associated complex, SKA) another subunit SKA2, in vitro and in vivo result of study all shows, SKA1 and SKA2 interacts and forms stable complex body, necessary (Hanisch A. for the stable of SKA2 and the location of SKA albumen in kinetochore and microtubule, Sillje HHW, Nigg EA.Timely anaphase onset requires a novelspindle and kinetochore complex comprising Ska1 and Ska2.EMBO J.2006, 25:5504-5515.).SKA complex body is most important for mitotic division, and all chromosomal kinetochores can be made all to be arranged in equatorial plate plane, and this is very necessary for guaranteeing the distribution of karyomit(e) equalization and maintaining Genome stability.Mitosis anaphase, karyomit(e) shifts to the two poles of the earth under the effect of spindle body kinetochore microtubule, and causes LC-PolScope image system reticent, and SKA1 complex body is also necessary albumen in this process.But in research at that time, the effect of SKA1 in chromosome segregation is not set forth clear.Report on Dev Cell and EMBO J magazine in 2009 has been set forth SKA1 complex body and played function on kinetochore and microtubule interface; and with microtubule direct effect; microtubule is formed oligomeric assembly; move along microtubule in a kind of mode of separating poly-coupling; chromosomal motion (Welburn JPI during participating in mitotic division; Grishchuk EL; Backer CB, et al.The human kinetochore Ska1 complexfacilitates microtubule depolymerization-coupled motility.Dev Cell 2009; 16:374-385.).
Genome research shows; 18q21.1 residing for SKA1 gene (Crowther-Swanepoel D relevant to the generation of chronic lymphocytic leukemia; Broderick P; Di Bernardo MC; et al.Common variants at 2q37.3; 8q24.21,15q21.3 and 16q24.1 influence chroniclymphocytic leukemia risk.Nature genetics 2010; 42:132-136.).This means that SKA1 can participate in the malignant proliferation of tumour cell by the mode of adjustment mitotic division process, cell cycle progress.In addition, resolve in the research of SKA1 function initial, process cell with microtubule depolymerization medicine nocodazole (nocodazole) and colchicine (colchicine), find that the water accumulation pancake of SKA1 in kinetochore is low; To the cell blocked during mitotic division, add nocodazole process, SKA1 and microtubule can be caused successively to depart from from kinetochore; On the contrary, when cell eliminates the process of nocodazole, the location of SKA1 albumen on kinetochore is recovered, and accordingly, spindle body is formed again.And microtubule stabilizer taxol (taxol); do not affect the location (SauerG of SKA1 on kinetochore; Korner R, Hanisch A, et al.Proteome analysis of the human mitotic spindle.Mol Cell Proteomics 2005; 4:35-43.).These researchs have all pointed out SKA1 may affect some antitumor drug susceptibility.But the report do not had at present about SKA1 and chemotherapy resistance, understands the function of SKA1 albumen in osteosarcoma and the impact on initial drug-resistant, has very strong value for clinical application.
Reverse transcription PCR, or claim reverse transcription PCR (reverse transcription-PCR, RT-PCR), be a kind of widespread use mode of polymerase chain reaction (polymerase chain reaction, PCR).In RT-PCR, a RNA chain is reversed record becomes complementary DNA, then carries out DNA cloning as template by PCR.This technology has broad application prospects in medical diagnosis on disease field.
Summary of the invention
Therefore, the technical problem to be solved in the present invention is exactly in the clinical diagnosis of tumour initial drug-resistant and treatment, lack the molecular diagnostic markers thing of effective predicting tumors initial drug-resistant and the molecular target for the treatment of tumour initial drug-resistant for current, a kind of effective solution is provided, namely one group effectively can be suppressed the siRNA of SKA1 genetic expression, the target sequences of described siRNA effect and can detect the reverse transcription PCR primer of SKA1 genetic expression and their application in preparation or screening antineoplastic drugs from tissue and cell.
The present invention solves the problems of the technologies described above one of technical scheme taked: a kind of SKA1 gene small molecule disturbance ribonucleic acid (siRNA) target DNA of separation, and wherein said target DNA is:
(1) DNA of continuous 15 ~ 27 Nucleotide composition on SKA1 encoding gene;
(2) any DNA in SEQ ID NO:1 ~ SEQ ID NO:4; Or
(3) DNA that the polynucleotide of hybridizing under stringent hybridisation conditions with (1) or the DNA described in (2) form, or with the DNA of its complementation.
SKA1 gene small molecule disturbance ribonucleic acid (siRNA) the target DNA molecular of separation of the present invention, is preferably made up of continuous 10 ~ 30 Nucleotide on SKA1 coding region gene, is more preferably the DNA of 15 ~ 27 Nucleotide compositions; Best, the target gene of SKA1 small molecule disturbance ribonucleic acid of the present invention is any DNA molecular in SEQ ID NO:1 ~ SEQ ID NO:4.
Wherein said hybridization conditions is classified according to the stringency degree of condition used during measurement hybridization.Stringency degree can the melting temperature(Tm) Tm of nucleic acid binding complex or probe be foundation, or with the salt of hybridization solution or ionic strength conditions for foundation.Described hybridization is preferably carried out at the standard conditions, can carry out according to the mode described in " molecular cloning ": Cold Spring Harbor Laboratory Press, the general scheme (Current Protocols in Molecular Biology) in molecular biology.More preferably, polymerized nucleoside acid hybridization can carry out in accordance with the following steps, and the film and the label probe that one are loaded with transcribed DNA to be measured or RNA molecule are hybridized in hybridization buffer.Hybridization buffer consist of 0.1wt%SDS, 5 wt% dextran glucosides, add 1/20 dilution inhibitor and 2 ~ 8 × SSC.20 × SSC is the solution of the citric acid composition of 3M sodium-chlor and 0.3M.Hybridization temperature is 50 ~ 70 DEG C.Cultivation several hours or after spending the night, clean film with cleaning buffer solution.Cleaning temperature is preferably room temperature, is preferably hybridization temperature.The composition of cleaning buffer solution is preferably 6 × SSC+0.1%SDS(wt) solution, be preferably 5 × SSC+0.1%SDS(wt).After having cleaned film with this cleaning buffer solution, just can by being identified DNA or RNA molecule by the mark on the probe of hybridizing in DNA or RNA molecule.
The present invention solves the problems of the technologies described above two of the technical scheme taked: the application of target DNA of the present invention in screening antineoplastic drugs.
The application of target DNA of the present invention in screening antineoplastic drugs is preferably as drug target.Described drug target refers to medicine effect binding site in vivo, selects to determine that novel active drug object point target is the top priority of new drug development.Rational drug design (rational drugdesign) can comprise the potential drug effect target position such as enzyme, acceptor, ionic channel, nucleic acid according to what disclose in life science, or the chemical structure characteristic of its endogenic ligand and natural substrate designs drug molecule, to find that selectively acting is in the new drug of target spot.By selection and the utilization of drug target, greatly can improve the efficiency of screening antineoplastic drugs, shorten the cycle of antitumor drug research.
The present invention solves the problems of the technologies described above three of the technical scheme taked: a kind of recombinant vectors, and wherein said recombinant vectors comprises target DNA of the present invention or comprises any sequence in SEQ ID NO:5 ~ SEQ IDNO:8.
Wherein said target DNA is comprised the DNA molecular of synthetic or to be increased from genome the DNA molecular be separated to by technology such as PCR.Recombinant vectors of the present invention preferably comprises any sequence in SEQID NO:5 ~ SEQ ID NO:8.
Wherein said recombinant vectors is selected from the carrier derived by retrovirus of this area routine.The carrier that described virus derives comprises lentiviral vectors, adenovirus carrier, adenovirus related vector, herpesvirus vector or vaccinia virus vector etc., the preferred lentiviral vectors of the present invention.The advantage of lentiviral vectors is that they can make the DNA of coding siRNA be incorporated in the genome of host cell, produced the clone that specific gene is prevented by specificity, some virus vector can be used for transformant in body, thus can manipulate directly in body and the genetic expression of whole biology.
Lentiviral vectors is mainly based on human immunodeficiency virus (HIV), by removing the virulent gene transformations such as env, vif, vpr, vpu, replace the coating of HIV-1 to pack with vesicular stomatitis virus G glycoprotein, host range is wide, can increase the titre of virus.The virulent gene of lentiviral vectors is deleted and replaced by foreign gene, and belong to pseudotype virus, and can not infect other cell again after this virus infected cell, biological safety is high.Lentiviral vectors all has infection ability to somatoblast and Unseparated Cell, and can longer-term is stable in vivo expression.The present invention's lentiviral vectors used is selected from the lentiviral vectors of this area routine, is preferably pFH1UGW carrier.
The present invention solves the problems of the technologies described above four of the technical scheme taked: a kind of small molecule disturbance ribonucleic acid (siRNA) suppressing SKA1 genetic expression, wherein said siRNA comprises just RNA fragment and antisense RNA fragment, described just RNA fragment comprises the RNA molecule of target DNA encoding described above, and described just RNA fragment and antisense RNA fragment complementaryly can form double stranded rna molecule.
SiRNA of the present invention is a kind of oligo rna molecule (length is generally at 21 ~ 25 Nucleotide).The major function of siRNA is the silence exciting target mRNA complementary with it.
SiRNA of the present invention comprises just RNA fragment and antisense RNA fragment, and the complementary pairing effect that described just RNA fragment and antisense RNA fragment pass through complementary base to each other forms double-stranded region.When just RNA fragment and antisense RNA fragment are positioned at different RNA chains, form double stranded rna molecule; When just RNA fragment and antisense RNA fragment are positioned at same RNA chain, then form the single strand RNA molecule with neck ring structure.Small molecule disturbance ribonucleic acid of the present invention (siRNA) length is for being preferably 8 ~ 50 Nucleotide, and between its sense fragment and antisense fragments, the base pair of complementary region is preferably 15 ~ 18 base pairs.
SiRNA of the present invention is preferably: any sequence of SEQ ID NO:5 ~ SEQ ID NO:8 and the RNA coded by complementary sequence, described siRNA comprise the formation RNA molecule of double-strand or the RNA molecule of strand.
Ribonucleic acid molecule (DNA) described in the present invention or DNA molecules (RNA) are by the mode of synthetic or obtained by the mode from genome amplification, and its method is the method that this area routine uses.
SiRNA of the present invention comprises the double-chain interference RNA (dsRNA) of synthetic, processes the siRNA obtained after transfectional cell in cell by Dicer enzyme system; By the siRNA that synthetic directly obtains; Or by building corresponding lentiviral vectors, the siRNA that continuous expression obtains in target cells.
The present invention solves the problems of the technologies described above five of the technical scheme taked: a kind of lentiviral particle, and wherein said lentiviral particle comprises recombinant vectors of the present invention.
Described lentiviral particle (Lentivirus) is by HIV-1(human immune deficiency I C-type virus C) based on the gene therapy vector that grows up.Distinguish general retroviral vector, it all has infection ability to somatoblast and Unseparated Cell.
Lentiviral particle is preparation method preferably comprise the following steps: be building up in lentiviral vectors by the object fragment that siRNA disturbs, then with package carrier cotransfection in eukaryotic cell, described eukaryotic cell is preferably 293T cell, after cultivating, carry out the recovery purifying of slow virus, obtain packaged lentiviral particle.
The present invention is by the reticent SKA1 gene of siRNA technology, one preferably example comprise the steps: first according to the sequence that the mRNA designated rna of SKA1 gene disturbs, then the DNA molecular of chemical complete synthesis this RNA molecule of coding, this DNA is inserted in plasmid, the Transfected Recombinant Plasmid 293T cell obtained, is packaged into recombinant slow virus.ShRNA(short hairpinRNA, the shRNA of this recombinant slow virus) in expression cassette containing siRNA encoding sequence of the present invention.Then for transfection tumor cell.After recombinant slow virus enters cell, following steps may be have passed through: utilize reversed transcriptive enzyme to transcribe out cDNA, then will recombinate in cellular genome containing cDNA of the present invention, utilize the enzyme system of host cell, transcribe out the shRNA for SKA1 gene of the present invention, the Dicer of SKA1shRNA and RNaseIII ribozyme family of the present invention combines, and is cut into siRNA of the present invention.The RNA that siRNA and several albumen form subsequently induces silencing complex (RNA-induced silencing complex, RISC) to combine, and untwists into strand, and dominates RNAi effect by this complex body.After RISC is activated, activated form RISC by becoming the siRNA of strand to guide, to be combined on SKA1 gene mRNA sequence-specific and to cut off SKA1 gene mRNA, the specific cleavage of initiation SKA1 gene mRNA.
The present invention solves the problems of the technologies described above six of the technical scheme taked: a kind of cell model of SKA1 gene silencing, described cell model comprises lentiviral particle of the present invention.
Cell model of the present invention is preferably eukaryotic cell, is more preferably tumour cell, preferably human osteosarcoma cell or colorectal cancer tumour cell.The preparation method of the cell model of SKA1 gene silencing of the present invention preferably comprises lentiviral particle transfecting eukaryotic cells of the present invention.
Wherein said transfection method is this area ordinary method, as DEAE-dextran method, and calcium phosphate method, cationic-liposome method, cationic polymers method, virus-mediated methods, biological particles passes method (particle gun Particle bombardment), microinjection, electroporation etc., preferably phosphoric acid calcium method of the present invention.Packaged lentiviral particle is transfected in clone, screens, obtain the gene silencing cell model of genetic stability.Wherein said clone is preferably eukaryotic cell lines, the preferred human osteosarcoma cell of the present invention, straight colon tumor cell.
One preferred embodiments of the preparation method of the cell model of SKA1 gene silencing of the present invention comprises: will pack successful recombinant slow virus and infect human tumor cells, then screen with tetracycline, the tumor cell clone of picking screening, detects the situation of the SKA1 protein content of different tumor cell clones by western-blot method.Result shows that the DNA sequence dna of code book invention siRNA is successfully recombinated in tumor cell gene group, and tentative confirmation siRNA sequence of the present invention can suppress the expression of SKA1 gene.Then the tumor cell clone that picking SKA1 protein content is lower, after continuous passage 2 generation, 4 generations, 6 generations, 8 generations, extract tumour cell mRNA with Trizol, semiquantitive RT-PCR analyzes the degraded situation of SKA1mRNA in tumour cell.Show that SKA1siRNA of the present invention can effectively degrade the mRNA of tumour cell SKA1 gene.Extract the albumen in the tumor cell clone of go down to posterity 6 times and 8 times, with the content of SKA1 albumen in western-blot method detection cell, show that siRNA sequence of the present invention can the expression of stabilization checking SKA1 gene.
The siRNA of SKA1 gene of the present invention can effectively degrade the mRNA of SKA1 gene, thus suppresses the expression of SKA1 gene.The present invention has successfully suppressed the expression of SKA1 gene with RNA perturbation technique, obtain the cell model of SKA1 gene silencing.
Tumor cell culture method, the preservation of cell model of the present invention and this area routine, activate, go down to posterity the same, usually with the DMEM substratum of 10% serum, 37 DEG C, containing 5%CO
2cell culture incubator in cultivate, with containing 20% serum, 10%DMSO DMEM substratum as frozen storing liquid freeze-stored cell.Digest with the cell dissociation buffer containing 0.25% pancreatin and 0.02%EDTA.
The present invention solves the problems of the technologies described above seven of the technical scheme taked: the application of cell model in screening antineoplastic drugs of SKA1 gene silencing of the present invention.
The application of cell model in screening antineoplastic drugs of described SKA1 gene silencing preferably comprises the following steps:
(1) drug candidate is made to contact with the tumour cell of SKA1 gene silencing;
(2) number of tumour cell is tested;
(3) drug candidate that tumor number is declined is selected.
The present invention's utilization does not carry out the Common tumors cell of SKA1 gene silencing as a control group.According to the present invention, described tumour cell preferably comprises human osteosarcoma cell or colorectal cancer tumour cell.The cell model utilizing the present invention to set up can carry out the research of tumour initial drug-resistant mechanism and tumor proliferation and amplification aspect.
The present invention solves the problems of the technologies described above eight of the technical scheme taked: small molecule disturbance ribonucleic acid of the present invention (siRNA) is preparing the application in antitumor drug.
Experiment confirms that SKA1 gene plays an important role in the initial drug-resistant process of tumour cell.After lentiviral particle containing SKA1-siRNA has infected osteosarcoma initial drug-resistant cell strain, confirm that the mRNA of endogenous SKA1 gene and protein level all significantly reduce by quantitative fluorescent PCR and immunoblot experiment.After endogenous SKA1 expresses and is suppressed, multiplication capacity, the tumorigenesis ability of osteosarcoma initial drug-resistant cell strain cell all significantly reduce, and greatly strengthen the susceptibility of antitumor drug.Small molecule disturbance ribonucleic acid of the present invention (siRNA) is applied to preparation and the screening of antitumor drug, preferably as a kind of sensitizer of antitumor drug.Application of the present invention preferably comprises a kind of pharmaceutical composition, and described pharmaceutical composition at least comprises a kind of small molecule disturbance ribonucleic acid of the present invention (siRNA) as activeconstituents and the pharmaceutically acceptable carrier of one.
Wherein said pharmaceutical composition preparation method preferably takes the method for this area routine, using siRNA of the present invention as activeconstituents, makes various formulation with pharmaceutically acceptable carrier.Wherein said carrier is the pharmaceutical carrier of this area routine, as weighting agent, thinner and vehicle etc.In various preparation, the weight content of activeconstituents is preferably 0.1% ~ 99.9%, and preferred weight content is 0.5 ~ 90%.
The present invention solves the problems of the technologies described above nine of the technical scheme taked: a kind of reverse transcription PCR primer of SKA1 gene.
The reverse transcription PCR primer molecule of SKA1 gene of the present invention comprises single stranded DNA, by external synthetic or be such as separated the method such as amplification by other routine techniquess of this area from genome and prepare and obtain.
Primer of the present invention is one section of oligomerization single stranded DNA or RNA molecule, and can be combined in region complementary with it in nucleic acid chains, its merit is the starting point of nucleotide polymerization effect, and nucleic acid polymerase can synthesize new nucleic acid chains by its 3 ' end.The primer of external engineer is widely used in polymerase chain reaction, order-checking and probe synthesis etc.The present invention also provides the application of reverse transcription PCR primer molecule in diagnosing tumor of described SKA1 gene.Described application one preferred embodiments is: with the RNA extracted in sample tissue or cell for template, utilize the reverse transcription PCR primer molecule of SKA1 gene of the present invention, reverse transcription synthesis cDNA, be template amplification target fragment again with cDNA, detect the expression amount change of SKA1 gene in tissue samples or cell, thus the development condition of diagnosing tumour or tumour cell.
The raw material that the present invention is used or reagent except special instruction, all commercially.
Compared to prior art, beneficial effect of the present invention is as follows: the present invention devises the reverse transcription PCR primer for SKA1 gene, RNA interfered target sequence, builds corresponding SKA1 shRNA expression vector, and wherein siRNA significantly can lower the expression of SKA1 gene at mRNA level in-site and protein level.Use slow virus to carry rna interference vector pFH1UGW-SKA1-siRNA-1 as genetic manipulation instrument the RNA interference sequence for SKA1 gene can efficiently be imported human osteosarcoma cell Saos-2, SF-86 and Human colorectal cancer cells RKO target, the expression level of remarkable reduction SKA1 gene, significantly improve the chemotherapy drug susceptibility of above-mentioned tumour cell, make the multiplication capacity of its initial drug-resistant cell strain cell, tumorigenesis ability all significantly reduces, and is one of potential clinical non-operative treatment mode of osteosarcoma and colorectal carcinoma.The reverse transcription PCR primer of SKA1 gene provided by the invention, this primer by detecting the expression amount change of SKA1 gene in cell or tissue, can be diagnosed tumour.
Accompanying drawing explanation
Below in conjunction with accompanying drawing, characteristic sum beneficial effect of the present invention is described.
Fig. 1 is Vector map.
Fig. 2 is siRNA positive clone identification collection of illustrative plates.
Fig. 3 is MTX drug sensitive test result.
Fig. 4 is IFO drug sensitive experiment result.
Fig. 5 is fluorescent quantitative PCR result histogram.
Embodiment
Further illustrate the present invention by embodiment below, but the present invention is not limited.The experimental technique of unreceipted actual conditions in the following example, usually conveniently condition, or according to the condition that manufacturer advises." room temperature " described in embodiment refers to the temperature of carrying out the operation room tested, and is generally 25 DEG C.
Embodiment 1 designs for the siRNA of SKA1
By the online siRNA design software of Invitrogen, choose four siRNA sequences that Website Evaluation is higher.By NCBI website, (Blast analysis) is compared to siRNA sequence.Find that these four siRNA sequences do not have homology significantly with other genes except SKA1.Article four, for the siRNA sequence of SKA1 in table 1.
The siRNA effect target sequences of table 1SKA1 gene
Numbering | Sequence numbering | Sequence |
siRNA-1 | SEQ ID NO.1 | GGAGATGAGATCATTGTAA |
siRNA-2 | SEQ ID NO.2 | GAGGACTTACTCGTTATGTTA |
siRNA-3 | SEQ ID NO.3 | CCGCTTAACCTATAATCAAAT |
siRNA-4 | SEQ ID NO.4 | GGGAGGACTTACTCGTTATGTTA |
Embodiment 2 builds the carrier containing SKA1-siRNA
2.1 molecule synthesis
According to the sequence in above table, by positive-sense strand and the antisense strand of Shanghai Sheng Gong biotech firm difference composite coding siRNA.Use ddH
2o is by for subsequent use to the concentration of 100 μMs for the serial dilution of synthesis.
The sequence of 4 the siRNA positive-sense strands wherein synthesized is respectively:
1、(SEQ ID NO.5):
5’-CTAGCGGAGATGAGATCATTGTAATTCA AGAGATTACA ATGATCTCATCTCCTTTTTTGGAATTAAT-3’;
2、(SEQ ID NO.6):
5’-CTAGCGAGGACTTACTCGTTATGTTATTCAAGAGATAACATAACGAGTAAGTCCTCTTTTTTGGAATTAAT-3’;
3、(SEQ ID NO.7):
5’-CTAGCCCGCTTAACCTATAATCAAATTTCAAGAGAATTTGATTATAGGTTAAGCGGTTTTTTGGAATTAAT-3’;
4、(SEQ ID NO.8):
5’-CTAGCGGGAGGACTTACTCGTTATGTTATTCAAGAGATAACATAACGAGTAAGTCCTCCCTTTTTTGGAATTAAT-3’。
The sequence of 4 the siRNA antisense strands wherein synthesized is respectively:
5、(SEQ ID NO.9):
5’-TAATTCCAAAAAAGGAGATGAGATCATTGTAATCTCTTGAATTACAATGATCTCATCTCCG-3’
6、(SEQ ID NO.10):
5’-TAATTCCAAAAAAGAGGACTTACTCGTTATGTTATCTCTTGAATAACATAACGAGTAAGTCCTCG-3’
7、(SEQ ID NO.11):
5’-TAATTCCAAAAAACCGCTTAACCTATAATCAAATTCTCTTGAAATTTGATTATAGGTTAAGCGGG-3’
8、(SEQ ID NO.12):
5’-TAATTCCAAAAAAGGGAGGACTTACTCGTTATGTTATCTCTTGAATAACATAACGAGTAAGTCCTCCCG-3’
Each component, according to following ratio, mixes by 2.2 cycle of annealings:
Solution | Volume |
10 × annealing buffer | 5μl |
Positive-sense strand | 5μl |
Antisense strand | 5μl |
H 2O | 35μl |
According to following program, carry out annealing reaction
2.3 enzymes are cut
The carrier used in the present invention is that pFH1UGW(is see " Fasano CA; Dimos JT; Ivanova NB; et al.shRNA knockdown of Bmi-1reveals a critical role for p21-Rbpathway in NSC self-renewal during development [J] .Cell Stem Cell, 2007Jun7.1 (1): 87-99 ").The structure of pFH1UGW is shown in Fig. 1.
According to following table, each component is mixed.
Carrier double digestion (wherein damping fluid 1 and PacI/NheI enzyme all come from NEB company)
Carrier | 5μl |
Water | 11.8μl |
10 × damping fluid 1 | 2μl |
100×BSA | 0.2μl |
PacI | 0.5μl |
NheI | 0.5μl |
Ligation (ligase enzyme is purchased from NEB company)
Carrier | 0.5μl |
Annealing reaction product | 7.5μl |
10 × connect damping fluid | 1μl |
T4 ligase enzyme | 1μl |
Room temperature connects 1 hour.
2.4 transform
1) 50 μ l competence Escherichia coli HB101 cells are taken out, and be placed in thawed on ice;
2) 5 μ l are connected products to join in 50 μ l competent cells, and be placed in and hatch 30 minutes on ice;
3) be placed in 42 DEG C of water-baths by containing the competent cell connecting product, hatch 90 seconds; Then be placed on ice, 3 minutes;
4) in pipe, add the LB substratum of 900 μ l antibiotic-frees; 37 DEG C, 200rpm, hatches 45 minutes;
5) 4000rpm, centrifugal 2 minutes;
6) abandon supernatant, then precipitation blown and beaten gently and after suspending, be added drop-wise to LB solid culture primary surface;
7) with spreading rod, solution is smoothened in media surface, and be placed in 37 DEG C of incubators, cultivate 12 ~ 16 hours.
2.5 clone bacterium liquid PCR qualifications
1) select single colonies and cultivate 4 hours in 3ml LB substratum, 250rpm;
2) according to following ratio, each component is mixed.
Wherein 5 ' primer: 5 '-GACAAATGGCAGTATTCATCC-3 ' (SEQ ID NO.13);
3 ' primer: 5 '-ATTTGCATGTCGCTATGTGT-3 ' (SEQ ID NO.14).
2×PCR Mix | 7.5μl |
H 2O | 4.5μl |
Bacterium liquid | 2μl |
5 ' primer | 0.5μl |
3 ' primer | 0.5μl |
Note: in the present embodiment, uses the Taq PCR MasterMix series product of Tian Gen company.
Reaction conditions:
3) by electrophoresis, qualification positive colony (as shown in Figure 2).
2.6 extracting plasmid DNA order-checkings in a small amount
The little extraction test kit of the plasmid of Tian Gen company is adopted in the present embodiment.
1) column equilibration step: the centrifugal 1min of the balance liquid BL adding 500 μ l in adsorption column CP3,12,000rpm, outwells the waste liquid in collection tube, is placed back in collection tube by adsorption column.
2) get the bacterium liquid of 2ml incubated overnight, add in centrifuge tube, use desk centrifuge, the centrifugal 1min of 12,000rpm, absorbs supernatant as far as possible.
3) in the centrifuge tube leaving bacterial sediment, add 250 μ l solution P1, use the thorough suspended bacterial precipitation of pipettor.
4) in centrifuge tube, add 250 μ l solution P2, leniently spin upside down and make the abundant cracking of thalline for 8 times.
5) in centrifuge tube, add 350 μ l solution P3, leniently spin upside down 8 times immediately, fully mix.The centrifugal 10min of 12,000rpm.
6) transfer in adsorption column CP3 by the supernatant liquor pipettor that previous step is collected, centrifugal 1 minute of 12,000rpm, outwells the waste liquid in collection tube, adsorption column CP3 is put into collection tube.
7) in adsorption column CP3, add 500 μ l protein liquid removal PD, centrifugal 1 minute of 12,000rpm, outwells the waste liquid in collection tube, is placed back in collection tube by adsorption column CP3.
8) in adsorption column CP3, add 600 μ l rinsing liquid PW, centrifugal 1 minute of 12,000rpm, outwells the waste liquid in collection tube, adsorption column CP3 is put into collection tube.
9) repetitive operation step 8.
10) adsorption column CP3 is put into collection tube, centrifugal 2 minutes of 12,000rpm, the remaining rinsing liquid in adsorption column is removed.
11) adsorption column CP3 is placed in a clean centrifuge tube, the middle part to adsorption film drips 50 μ l H
2o.Room temperature places 2 minutes, centrifugal 2 minutes of 12,000rpm.Plasmid solution is collected in centrifuge tube.
Get the little plasmid taken out of 5 μ l to deliver to company and check order, determine that SKA1-siRNA sequence has correctly been inserted in pFH1UGW carrier.
Embodiment 3 expresses the virus packaging of SKA1-siRNA
Take out in 3.1 plasmids (in take out test kit purchased from Pu Luomaige biotech firm, article No.: A7640)
1) get the LB substratum (containing appropriate microbiotic) that the fresh bacterium liquid of 50 μ L is inoculated into 15 ~ 50mL, 37 DEG C shake cultivation 14 ~ 16 hours.Under room temperature 5,000 × g centrifugal 10 minutes, collect thalline, and suck supernatant as much as possible.
2) BufferA1 that 2.5mL has added RNase A is added, Eddy diffusion thalline.
3) add 2.5mL Buffer B1, reverse 5 ~ 10 times lightly to mix, then leave standstill and clarify to solution thickness for 2 ~ 5 minutes.
4) add 3.0mL Buffer C1, reverse 5 times immediately, firmly rock 3 ~ 5 fully mixings with hand, now occur white flock precipitate.
5) centrifuge tube is gone to supercentrifuge, at room temperature 14,000g centrifugal 10 minutes; Supernatant liquor after careful absorption is centrifugal, in 15mL pipe, adds 3.0mL 100% ethanol, shakes up immediately, needs the centrifugal DNA of mistake at once to reclaim post.
6) shift 6.0mL lysate/collection tube immediately in the DNA post of band collection tube, under room temperature 5,000g centrifugal 1 minute, outwell the waste liquid in collection tube, centrifugal column is placed back in collection tube; Repeat this step until all solution is by DNA post.
7) in centrifugal column, add 4mL 70% ethanol, under room temperature 5,000g centrifugal 1 minute, outwell the waste liquid in collection tube, centrifugal column is placed back in collection tube.
8) put back in supercentrifuge by centrifugal column, under room temperature, 5,000g uncap centrifugal 10 minutes.
9) gone to by centrifugal column in a new 15mL centrifuge tube, the center to DNA post film adds the ddH of 0.5mL
2o(pH is between 7.0 ~ 8.5) or dissolve damping fluid, room temperature places 1 minute, and centrifugal 5 minutes of 5,000g, with wash-out plasmid DNA.
10) DNA concentration and purity: DNA concentration (μ g/mL)=OD
260× 50 × extension rate.
3.2 plasmid co-transfection
1) plasmid concentration and purity is detected: extracting obtains the good plasmid of purifying, determines plasmid concentration (1.28 μ g/ μ l, OD
260/ OD
280show without protein contamination between 1.75 ~ 2.0), and purity (0.8% ~ 1.0% agarose gel electrophoresis result display plasmid is superhelix single tape, pollutes without RNA).
2) plating cells: by collected by trypsinisation 293T cell (293T purchased from life science institute cellular resources center, Chinese Academy of Sciences Shanghai, article No.: GNHu17), with (perfect medium: DMEM+10%FBS after the dilution of suitable perfect medium.Substratum DMEM, purchased from Hyclone company, article No. is: SH30243.01B; Foetal calf serum purchased from GIBCO company, article No.: 10099141; Microbiotic is purchased from Hyclone company, and article No.: SV30010, working concentration penicillin is 100U/mL, and Streptomycin sulphate is 100 μ g/mL) with 1 × 10
5to 4 × 10
5cell/cm
2density inoculating cell on Tissue Culture Dish.293T cell is placed in containing 5%CO
237 DEG C of incubators in hatch 8 ~ 24h, when cell attachment completely after namely start transfection.Before transfection, 2h changes liquid (replacing old substratum with fresh perfect medium).
3) calcium phospate-DNA precipitate is prepared: DNA and CaCl
2mixing.In 60mm tissue culture dishes, react cumulative volume is 500 μ l.In aqua sterilisa, add plasmid DNA (3 ~ 5 μ g), then add 31 μ l 2MCaCl
2, make three's cumulative volume reach 250 μ l, mixing.
4) by plasmid and CaCl
2mixture dropwise add 250 μ l(equal-volumes) 2 × HBS buffered soln.Flick tube wall simultaneously, make often to be added dropwise to rear timely mixing.After leaving standstill 20min, the calcium phosphate-DNA suspension of this 500 μ l is dropwise added in the cell culture medium of above-mentioned monolayer cell, shake plate mixing gently.
5) be placed in containing 5%CO
237 DEG C of incubations.Cultivate (8 ~ 24h) after for some time and suck substratum with DNA precipitate, add the perfect medium of 5ml 37 DEG C of preheatings, continue cell to place incubation, after cultivating 24 ~ 48h, observe the expression of albumen, and collection is viral.
3.3 viral purification
1) the 293T cell culture supernatant of 48h after transfection is collected;
2) the centrifugal 10 ~ 15min of refrigerated centrifuge 3000 ~ 4000g is used, removing cell debris;
3) use 0.45 μm of filter filtration cell culture supernatant, and be dispensed in 40ml ultracentrifugation pipe;
4) viral crude extract sample is joined in filtering cup, build lid; Filtering cup is inserted in collection tube; This filtration unit is the plus-20 centrifugal filter device of MILLIPORE;
5) assemble after strainer tube weight adjustment, put into whizzer;
6) the centrifugal 10 ~ 15min of 3000 ~ 4000g on refrigerated centrifuge;
7) take out centrifugal device after centrifugal end, filtering cup is separated with filtered liquid collection cups below;
8) filtering cup is tipped upside down on sample collection cup;
9) the centrifugal 2 ~ 5min of refrigerated centrifuge 500 ~ 1000g is used; Centrifuge Cup is removed from sample collection cup; In sample collection cup, liquid is viral purification concentrated solution.
3.4 titres detect
1) crude extract titer determination:
A) viral supernatants 4 DEG C preservation is collected;
B) carry the day before yesterday at 96 orifice plate middle berth 293T cells, every porocyte number is: 2 × 10
4individual, volume is 100 μ l;
C) virus stock solution used is added in cell according to 100 μ l, 50 μ l, 20 μ l, 10 μ l, 1 μ l;
D) infect after 3 days and observe fluorescence;
E) determine a scale virus (Virus Standard product are ordered from Niu En biotech firm) simultaneously, do 10 at every turn
8, 10
7, 10
6standard substance.
2) concentrating virus titer determination:
A) collect viral supernatants and carry out filtration and ultracentrifugation ,-80 DEG C frozen;
B) carry the day before yesterday at 96 orifice plate middle berth 293T cells, every porocyte number is: 4 × 10
4individual, volume is 100 μ l;
C) according to the expection titre of virus, prepare 7 ~ 10 aseptic EP pipes, often pipe adds 90 μ lopti-MEM;
D) get virus-4 to be measured DEG C to thaw, draw 10 μ l and join in the 1st pipe, get 10 μ l after mixing and join in the 2nd pipe.Continue a same operation to the last pipe;
E) choose required cell hole, suck 90 μ l substratum, add the viral solution that 90 μ l have diluted, put into incubator and cultivate;
F), after infecting 24h, add perfect medium 100 μ l, careful operation does not blow afloat cell;
G) infect after 3 days, observe fluorescence.Fluorocyte number reduces with the increase of extension rate;
Illustrate:
Pipe marks | 1st pipe | 2nd pipe | 3rd pipe | ...... | 7th pipe | 8th pipe |
Either stock virus amount | 1E+1μl | 1E+0μl | 1E-1μl | ...... | 1E-5μl | 1E-6μl |
H) titre calculates: according to the fluorescence situation of actual observation, suppose to observe 3 cells with fluorescence in the 8th pipe, illustrate in this hole to have 3 infestation with virus particles cell at least, then the titre of this virus equals cell count with fluorescence divided by virus stock solution used amount, the virus stock solution used amount of the 8th pipe is 1E-6 μ l, so titre=3/(1E-6)=3E+6, unit is TU/ μ l, namely equals 3E+9TU/ml.By above-mentioned virus titer method of calculation, the virus titer of known this packaging SKA1-siRNA is 5 × 10e8 TU/ml.
On the impact of the resistance of drug-resistant cell strain after embodiment 4SKA1 gene expression inhibition
4.1 key instruments and reagent
Cellomics(Thermo);
CO
2incubator (MCO-15A SANYO);
Inverted microscope (XDS-100 Shanghai Cai Kang opticinstrument company limited);
Super clean bench (EQR/GL-41ESCO);
Whizzer (TDL-50B pacifies booth);
SF-86 cell is osteosarcoma drug-resistant cell strain, for CCTCC NO:C201002(is see Chinese patent application CN201010110746.X).
MTX: methotrexate, derives from Shanghai Ke Xing laboratory equipment company limited, article No.: 100138;
IFO: ifosfamide, Shanghai Ke Xing laboratory equipment company limited, article No.: 100595.
4.2 experimental procedure
1) drug sensitive experiment
A) by contrast interference (control) virus, (described contrast virus is PSCN, the siRNA sequence comprised in this lentiviral vectors is TTCTCCGAACGTGTCACGT, not for the gene in any human body, for getting rid of the toxic action to cell itself brought by virus, this slow virus is purchased from Niu En biotech firm) and embodiment 3 gained the target sequences comprising SKA1 gene siRNA and can the lentiviral particle of expressing green fluorescent protein, infect SF-86 cell respectively, experiment comprises the following steps: 1, and cell spreads 12 orifice plates according to the density of 10%; 2, next day, change fresh culture; 3, adding polybrene to final concentration is 5 μ g/ml; 4, add lentiviral particle and the contrast virus of embodiment 3 gained; 5, three, change liquid maintain three days; 6, by fluorescent microscope, observation of cell efficiency of infection, efficiency of infection reaches 90%.
B) observation of cell after 4 days is infected, find the infected upper virus of most cells in each infected group, because virus vector there is GFP label protein, therefore after cell infection, GFP albumen can be expressed, namely by the strong and weak ratio height with expressing GFP cell of expression of GFP in fluorescence microscope cell, efficiency of infection is judged.
C) by after the enzymic digestion of each experimental group cell tryptase, perfect medium (same as above) re-suspended cell, spreads to 96 orifice plates.Often organize 8 multiple holes, every hole 100 μ l, after completing plate, puts 37 DEG C of 5%CO
2incubator is cultivated.
D) after cell attachment, each infected group is further divided into add MTX medicine (3 multiple hole), add IFO medicine (3 multiple hole), not dosing (2 multiple hole) three groups, add corresponding drug treating, MTX working concentration is 1 μ g/ml; IFO working concentration is 222 μ g/ml.
E) detect with CELLOMICS instrument respectively during dosing 24 hours, 48 hours, 72 hours and calculate the number of different treatment group cell respectively.
F) data processing
Calculate in dosing after 24 hours, 48 hours and 72 hours respectively, often organize the cell survival rate of cell under MTX and IFO drug effect that RNA disturbs slow virus infection:
Cell number when survival rate=medicine exists/without cell number during drug treating.
The survival rate of cell can reflect the susceptibility of tumour cell to medicine.By compare group (control) and RNA interference group, cell, to the change of drug susceptibility, analyzes the effect of this gene in cellular drug resistance.Utilize the change of the cell count of non-dosing group, the impact of analyzing gene on cell proliferation: cell count during 24h, as 1, calculates the ratio change of the cell count of 48h, 72h.
2) Effective target site strikes and subtracts checking
A) from 4 goal gene disturbance target points, screening obtains 2 target spots that drug susceptibility is increased and carries out striking the checking subtracting efficiency.
B) osteosarcoma drug-resistant cell strain SF-86 is infected respectively with the lentiviral particle comprising 2 siRNA target sequences (siRNA-1 and siRNA-2) of embodiment 3 gained and negative control virus (negative control virus is same as above), infect peptic cell after 4 days, centrifugal collecting cell precipitates.Described experimental procedure comprises: 1, and cell spreads 12 orifice plates according to the density of 10%; 2, next day changes fresh culture; 3, adding polybrene to final concentration is 5 μ g/ml; 4, add embodiment 3 gained lentiviral particle, described slow virus titre is 5 × 10e8TU/ml, and virion dilutes according to 1:500, and cell infection plural number is 10; 5, cell changes liquid maintain three days; 6, cell cultures passes through fluorescent microscope, observation of cell efficiency of infection > 90% on the 3rd day.
C) use lysate trizol lysing cell, extracted total RNA, reverse transcription becomes cDNA, carries out quantitative fluorescent PCR.Detect SKA1mRNA.
Wherein SKA1-5 primer: 5 '-GATGAGTTCAATGGTGTTCCTTC-3 ' (SEQ IDNO.15);
SKA1-3 primer: 5 '-CCTTTGGTATCCTTCGTTTCTTC-3 ' (SEQ IDNO.16).
D) analysis of fluorescence quantitative PCR result data (shown in table 2, Fig. 5).
The statistical study of table 2 fluorescent quantitative PCR result
4.3 experimental results:
1) drug sensitive experiment results and analysis
A) for after the RNA interference slow virus infection resistance SF-86 cell of the siRNA-3 target spot of SKA1 gene, cell increases the susceptibility of MTX, and the high expression level of this gene in SF-86 cell may (see figure 3) relevant to its medicine of resistance to MTX.Because SF-86 cell is drug-resistant cell strain, therefore this cell strain is without under drug condition and when having a MTX, and upgrowth situation is similar.
B) after embodiment 3 gained comprises the RNA interference slow virus infection resistance SF-86 cell of SKA1 gene siRNA-2, siRNA-3, siRNA-4 target spot, cell increases the susceptibility of IFO, and in SF-86 cell, the high expression level of SKA1 gene may (see figure 4) relevant to its medicine of resistance to IFO.
2) according to medicament sensitivity test, this experimental selection wherein drug susceptibility the most obvious siRNA-1 target spot of rising and siRNA-3 target spot carries out SKA1 gene inhibition validation verification.The result SKA1 gene inhibition successful (see table 2).After quantitative fluorescent PCR reaction, first we analyze the solubility curve of SKA1 and internal reference actin, and result illustrates that quantitative fluorescent PCR can increase SKA1 gene and internal reference actin specifically.By 2
-Δ Δ Ctmethod is analyzed, and can obtain conclusion: namely relative to the compared with control cells of virus-free infection, infected in the experimental group cell of the slow virus comprising SKA1-siRNA, the gene expression dose of SKA1 significantly reduces.
3) interpretation of result: SKA1 is the moiety of kinetochore, spindle fibre related complexes, centric formation and chromosomal cohesion when participating in mitotic division, and participates in the extension of actin and depolymerization has the function promoting cell mobility.But report be there is no for the function of this gene in tumour.The cells proliferation slowed down of siRNA-1 target spot in this experiment, siRNA-3 target spot increases MTX susceptibility, siRNA2,3,4 target spots increase IFO susceptibility.From the resistance mechanism of MTX and IFO two kinds of medicines, all synthesize with DNA and suppress relevant, show that they functionally have certain intersection.All in all, after changing the expression of gene, the responsive type of cell to IFO medicine more easily displays.
The reverse transcription PCR primer of embodiment 5SKA1 in osteosarcoma cell for the detection of SKA1 gene
Utilize SKA1 gene reverse transcription PCR primer provided by the invention, with the RNA extracted from osteosarcoma cell line for template reverse transcription synthesis cDNA, again with this cDNA for template amplification synthesis object fragment, the method can detect the expression level of SKA1 gene in osteosarcoma cell.
The reverse transcription PCR primer of embodiment 6SKA1 in osteosarcoma clinical pathology sample for the detection of SKA1 gene
Utilize SKA1 gene reverse transcription PCR primer provided by the invention, from osteosarcoma clinical pathology sample, extract RNA, and with this RNA for template reverse transcription synthesis cDNA, then be template with cDNA, amplification synthesis object fragment.The method can detect the expression level of SKA1 gene in osteosarcoma clinical pathology sample.
The all documents mentioned in the present invention are quoted as a reference all in this application, are just quoted separately as a reference as each section of document.In addition should be understood that those skilled in the art can make various changes or modifications the present invention after having read foregoing of the present invention, these equivalent form of values fall within the application's appended claims limited range equally.
Claims (1)
1. an anti-human osteosarcomatous small molecule disturbance ribonucleic acid, it is characterized in that, described small molecule disturbance ribonucleic acid is made up of just RNA fragment and antisense RNA fragment, described just RNA fragment is that described antisense RNA fragment is the complementary RNA molecules of this just RNA fragment by the RNA molecule of DNA sequence encoding shown in SEQ ID NO:1 in sequence table.
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